| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 1997063 | Molecular Cell | 2010 | 10 Pages |
SummaryTranslesion synthesis is an essential cell survival strategy to promote replication after DNA damage. The accumulation of Y family polymerases (pol) ι and Rev1 at the stalled replication machinery is mediated by the ubiquitin-binding motifs (UBMs) of the polymerases and enhanced by PCNA monoubiquitination. We report the solution structures of the C-terminal UBM of human pol ι and its complex with ubiquitin. Distinct from other ubiquitin-binding domains, the UBM binds to the hydrophobic surface of ubiquitin centered at L8. Accordingly, mutation of L8A, but not I44A, of ubiquitin abolishes UBM binding. Human pol ι contains two functional UBMs, both contributing to replication foci formation. In contrast, only the second UBM of Saccharomyces cerevisiae Rev1 binds to ubiquitin and is essential for Rev1-dependent cell survival and mutagenesis. Point mutations disrupting the UBM-ubiquitin interaction also impair the accumulation of pol ι in replication foci and Rev1-mediated DNA damage tolerance in vivo.
► UBM adopts a structural fold distinct from other ubiquitin-binding domains ► UBM binds to the hydrophobic surface of ubiquitin centered at L8 ► Mutation of ubiquitin-binding residues in UBM impairs pol ι foci accumulation ► Disruption of Rev1-ubiquitin interaction diminishes yeast survival and mutagenesis
